Production and characterization of bacterial cellulose by Rhizobium sp. isolated from bean root

Bacterial cellulose (BC) is a natural polymer renowned for its unique physicochemical and mechanical attributes, including notable water-holding capacity, crystallinity, and a pristine fiber network structure. While BC has broad applications spanning agriculture, industry, and medicine, its industrial utilization is hindered by production costs and yield limitations. In this study, Rhizobium sp. was isolated from bean roots and systematically assessed for BC synthesis under optimal conditions, with a comparative analysis against BC produced by Komagataeibacter hansenii. The study revealed that Rhizobium sp. exhibited optimal BC synthesis when supplied with a 1.5% glucose carbon source and a 0.15% yeast extract nitrogen source. Under static conditions at 30 °C and pH 6.5, the most favorable conditions for growth and BC production (2.5 g/L) were identified. Modifications were introduced using nisin to enhance BC properties, and the resulting BC-nisin composites were comprehensively characterized through various techniques, including FE-SEM, FTIR, porosity, swelling, filtration, and antibacterial activity assessments. The results demonstrated that BC produced by Rhizobium sp. displayed properties comparable to K. hansenii-produced BC. Furthermore, the BC-nisin composites exhibited remarkable inhibitory activity against Escherichia coli and Pseudomonas aeruginosa. This study contributes valuable insights into BC’s production, modification, and characterization utilizing Rhizobium sp., highlighting the exceptional properties that render it efficacious across diverse applications.


3D
Three Cellulose, a water-insoluble polysaccharide, is derived from various organisms, including animals, plants, algae, bacteria, and cell-free systems 1,2 .It stands out as the most prevalent renewable biopolymer within the biosphere, positioning it as a favorable candidate for the escalating need for biocompatible and environmentally sustainable applications.However, the rising demand for cellulose products derived from plants has led to heightened wood consumption, consequently exacerbating deforestation-a significant worldwide environmental conditions on BC structure and properties.The yield, structure, and morphology of hydrated BC were compared with those of BC produced by K. hansenii, a well-known efficient BC producer.The nanofibers generated in the selected media underwent characterization for various structural and physicochemical properties, including Fourier Transform Infrared spectroscopy (FTIR), Field-Emission Scanning Electron Microscopy (FE-SEM), water release rate (WRR), water-holding capacity (WHC), swelling, porosity, filtration, and antibacterial properties.The BC produced by Rhizobium sp.exhibited novel properties suitable for biomedical applications, such as scaffolds for tissue engineering and protein-based drug uptake and release.Furthermore, nisin was incorporated into the material to enhance the antimicrobial activity of the dehydrated BC composite, rendering it effective against various microorganisms, including Gram-positive and Gramnegative bacteria.In order to gain a deeper understanding of the material's properties, a detailed investigation was conducted into the various structural and physicochemical properties of both BC and BC-nisin composite membranes.Moreover, the in vitro antimicrobial activity of the BC-nisin composite membranes was evaluated.

Microbial strains
A strain of K. hansenii, ATCC 53582, was used for BC production.Escherichia coli and Pseudomonas aeruginosa from the culture collection of the Department of Biology, College of Science, University of Baghdad, Iraq, were used to determine the antibacterial activity of the composite membrane.

Media
A mannitol yeast extract agar (MYA), HS agar media, and their modifications (culture media, broth fermentation media, and production media) were used for BC production.Each medium was tailored to meet specific nutritional requirements and facilitate the desired metabolic activities of the organisms under study.Each medium was prepared according to established protocols and sterilized using appropriate techniques to maintain integrity and prevent contamination.

Plant material collection statement
Plant material collection adhered to institutional, national, and international regulations.Vicia faba is not classified as a protected or endangered species among wild plants in Iraq, hence necessitating no permissions for the research material collection.

Isolation and characterization of the microorganisms
The root nodules of V. faba plants were gathered from various farms in Aladamya, Baghdad city, Iraq, and placed in a sterile container.Healthy root nodules were carefully chosen, subjected to tap water to eliminate soil adhesion, and cleaned with distilled water.Sterilization was carried out using 95% ethanol and H 2 O 2 (4%) for a duration of 2 min, followed by maceration and a subsequent wash with sterile water for 3 min.Finally, the nodules underwent immersion in a 0.1% HgCl 2 solution for 2 min to establish a pure culture of Rhizobium sp. (Fig. 1).

Morphological identification of Rhizobium sp.
The extracted sample was taken from the suspension and placed on a glass slide for morphological identification and microscopic examination.Their shapes, cell forms, and morphological characteristics were studied using the Gram stain kit.The examination was conducted under a compound light microscope with an oil-immersion lens at 100× magnification.Simultaneously, culture characteristics were assessed by inoculating the suspension on MYA and allowing it to incubate at 25 °C for 3-5 days.The standard culture media consisted of 10 g mannitol, 1 g yeast extract, 0.5 g K 2 HPO 4 , 0.2 g MgSO 4 , 0.1 g NaCl, 0.1 g CaCO 3 , and 15 g/L agar, with an initial pH of 6.8.The resulting solution was transferred to a glass bottle with a 1-L capacity and autoclaved at 121 °C for 15 min 42,43 .
The collected samples were stored in sterile containers at 4 °C and underwent homogenization and serial dilution.Each dilution was spread on HS agar media (20 g/L glucose, 5 g/L yeast extract, 5 g/L peptone, 6.8 g/L Na 2 HPO 4 × 12H 2 O, 1.5 g/L citric acid, and 20 g/L agar, with an initial pH of 6.0), and incubated for 3 days at 30 °C.After incubation, a single colony was chosen, inoculated into 100 mL/250 mL (100 mL culture media within the 250 mL flask) HS broth media for seed culture, and incubated for 48 h at 30 °C.For BC production, 2% (v/v) of the strained broth was inoculated into 300 mL/500 mL (300 mL culture media within the 500 mL flask) HS broth fermentation media.The microbial cultures were then incubated in treated molasses prepared with 250 mL culture media within the 500 mL flask for 7 days at 30 °C under static conditions.Subsequently, colonies displaying Gram-negative staining and producing white cellulose pellets were selected for further analyses 44 .

Biochemical identification of Rhizobium sp.
The biochemical tests for the isolate of Rhizobium sp.included various assays performed on bacterial strains isolated from root nodules of the bean under investigation.These tests encompassed the Fluorescence Test 45 ,

Preparation of the BC composite membrane
The BC membrane was freeze-dried and shaped into circular forms with diameters of 1 cm.Nisin dispersions were prepared in 0.5% (v/v) acetic acid to achieve a final concentration of 1.5% (w/v) and stirred at 37 °C for approximately 3 h.The solution was then oven-dried.The resulting solution was filtered through a polyester cloth to eliminate residual insoluble particles.The BC-dried membrane pellicle was soaked in a nisin-acetic acid solution for 48 h at room temperature to produce a BC-nisin membrane.Various nisin concentrations (100, 200, 300, and 400 IU) were blended to create the BC composite membranes, named cellulose-nisin membranes (BC-Nis).

Determination of the optimal carbon source for BC production
The effect of carbon sources on cellulose production was studied using different substances such as maltose, fructose, and glucose at a concentration of 2% added individually to HS.

Determination of the optimal glucose concentration for BC production
The effects of different glucose concentrations were studied, and the best carbon source in the production media was between 0.5 and 3%.

Determination of the optimal nitrogen source for BC production
The effect of nitrogen sources on cellulose production was studied using different substances such as yeast extract, peptone, tryptone, NH 4 Cl, and (NH 4 ) 2 SO 4 at a concentration of 0.05% added individually to HS.The effects of different concentrations of yeast extract were studied, and the best source of nitrogen in the production media was found to be between 0.05 and 0.2%.

Environmental conditions pH value
Media with a pH between 5 and 7 were prepared to determine the optimum pH for cellulose production.The pH of the media is adjusted by adding concentrated hydrochloric acid to lower the pH or sodium hydroxide to raise the pH.Simultaneously, the source and concentration of the optimal carbon source and nitrogen concentration for optimal cellulose production were determined based on the results of the above experiments.

Temperature
The media were incubated at different temperatures from 25 to 35 °C (25 °C, 30 °C, and 35 °C), with a difference of 5 °C from one media to another, and inoculated with bacterial production.The optimal temperature for cellulose production was determined for 7 days, considering the optimal growth conditions from previous experiments.

Aeration
The experiment was conducted in a glass bottle, one filled with air and the other covered with a cotton lid.The following steps prevented contamination of the culture: (1) sterilization of microbiological instruments and media using a convection oven and autoclave; (2) working in a biosafety cabinet; (3) adjusting the incubator temperature to prevent unwanted growth of organisms.

Determination of the dry and wet weights of BC
For this purpose, the wet weight of the BC was determined after washing with distilled water.The dry weight was determined using a digital balance (GENIUS, Sartorius, Germany) with an accuracy of 0.001 g after drying 54 .

Determination of the thickness of BC membranes
Thickness measurements of the BC membranes were conducted using a digital micrometer (Mitutoyo, no.293-766; Tokyo, Japan).10 different points on each BC sample were selected for measurement, and the average values were calculated 55 .

Characterization of composite membrane FE-SEM analyzes
To examine the structural properties of the pure freeze-dried BC/K.h, and BC/K.h-Nis membranes, as well as BC/Rhiz and BC/Rhiz-Nis membranes, the BC membranes were fractured using liquid nitrogen, attached to a substrate with carbon tape, and coated with a thin layer of gold.The internal microstructure of the BC membranes, with a focus on the impregnation of nisin nanoparticles into the BC matrix, was observed using FE-SEM (Hitachi S-4800 and EDX-350 (Horiba), Tokyo, Japan) at an accelerating voltage of 10 kV at room temperature.
Fourier Transmission Infra-red Spectroscopy (FTIR) analyzes FTIR analysis of freeze-dried BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis samples were conducted using a BIO-RAD FTS-7PC FTIR spectrophotometer (Bio-Rad, Cambridge, MA).The experimental conditions for the FTIR measurements were set to a spectral range of 400-4000/cm and a resolution of 0.25/cm.Additionally, FTIR spectra of the pristine freeze-dried BC, BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis scaffold samples were analyzed using a Perkin-Elmer FTIR spectrophotometer (Perkin-Elmer, Hopkinton, Massachusetts, USA).The experimental conditions for these measurements were also set to a spectral range of 400-4000/cm and a resolution of 0.25/cm.The samples were thoroughly mixed with potassium bromide (KBr) pellets (IR grade; Merck, Germany) to facilitate the analysis.The resulting mixture was then used to obtain IR spectra, which were transferred to a computer for further spectral analysis.

The water holding capacity (WHC) and water release rate (WRR)
The water-holding capacities of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis composites were assessed using the sieve shaking method.The dried BC sheets were immersed in distilled water for an appropriate period to allow complete swelling.The plates were carefully removed from the storage containers using tweezers.Subsequently, the samples were placed in a sieve and shaken vigorously twice to eliminate any remaining surface water before weighing.The samples were then air-dried at room temperature, and their weights were recorded at various time intervals (45 h).To ensure complete moisture removal, the samples were dried in an oven at 60 °C for 24 h and then dried at room temperature.The water-holding capacity (WHC) of each sample was determined using the following formula 56 :

Mass of water removed during drying g Dry weight of cellulose sample g
The WRR was determined by measuring the initial weight of the cellulose samples.These samples were stored under ambient conditions for different durations and weighed periodically until a uniform dry weight was obtained 1 .

Porosity analyzes
The porosity of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis composites were determined using the previously developed method.To ascertain the porosity of BC, it underwent a 12-h immersion in distilled water at ambient temperature.The porosity percentage was calculated using the following formula 57 :

Swelling analyzes
Swelling abilities of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis composites were also investigated.The membranes were cut into 2 × 2 cm square shapes, dried to constant weight, and subsequently subjected to drying until a constant weight was achieved.After this, water elimination occurred, and the membranes were immersed in deionized water at room temperature 58 .The swelling ratio (SR%) was determined through the application of the following equation: W t represents the weight of the hydrogel in its swollen state, and W d indicates the hydrogel's weight when in its dried state.Swelling assessments were performed in triplicate.The average results were then calculated according to the method 59 .

Filtration analyzes
The filterability of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis composites were assessed by passing 100 mL of distilled water through samples dried at 70 °C for 4-6 h and determining the diameter.The time taken for the water to filter through each sample was determined as previously reported 60 .

Antibacterial activity of the composite membrane
To investigate the antibacterial activity of cellulose obtained from K. hansenii and Rhizobium sp., samples were treated with different nisin concentrations for 24 h.The zones of inhibition for E. coli and P. aeruginosa, cultivated on nutrient agar, were determined utilizing the disk diffusion method.BC membranes lacking nisin served as the control specimens.Subsequently, the agar plates were incubated at 30 °C for a duration of 48 h.The antibacterial activity was assessed by measuring the diameter of the inhibition zone surrounding the BC composite membrane, and the results were quantified in arbitrary units (mm).

Data analysis
Each measurement for every group was repeated 3 times (N = 3).The data were presented as the mean standard error for both the control and experimental groups.The experimental data were analyzed using IBM SPSS 24.0, and the statistical significance was determined at p ≤ 0.05.The graphs were generated using GraphPad Prism 9.3 (https:// www.graph pad-prism.cn/).

Results and discussion
Isolation and characterization of Rhizobium sp.
Rhizobium sp. was isolated from vital root nodules and subjected to a comprehensive identification procedure based on morphological, cultural, and microscopic characteristics.The morphological and cultural characteristics of the bacterial colonies were determined by analyzing their appearance on MYA.The colonies exhibited large, shiny, milky-white raised circular structures with a conspicuous mucoid surface texture.Microscopic analysis revealed that Rhizobium sp.exhibited typical Gram-negative rod-shaped bacterial characteristics.

Biochemical characterization and identification of Rhizobium sp.
The results of biochemical tests for the isolated Rhizobium sp.showed distinctive characteristics (Table 1).Rhizobium sp.colonies on MYA agar plates with Congo Red (CR) indicator displayed a light red color.The strain demonstrated the ability to produce oxidase and catalase enzymes but was negative for indole production, Voges-Proskauer, sodium citrate utilization, H 2 S production, urease, and gelatinase enzymes 61,62 .

Production and purification of BC by Rhizobium sp.
The ability of Rhizobium sp. to produce cellulose was investigated by culturing the isolate in HS media and determining the dry weight of the cellulose produced.The results showed that Rhizobium sp.produced cellulose with a dry weight of 2.5 g/L, which was visually manifested as a white pellicle layer on the surface of the HS media.Determination of the optimal carbon source for BC production Figure 2A illustrates the effects of different carbon sources on cellulose production by Rhizobium sp.The results showed that glucose had the highest cellulose productivity among the sugars.The amount of cellulose produced was 1.75 g/L, followed by maltose at 1.3 g/L and fructose at 0.3 g/L.Consequently, the subsequent experiments chose glucose as the optimal carbon source for cellulose production.
Fructose, a widely available and cost-effective sugar found mainly in industry and waste, has been suggested as the preferred carbon source for cellulose production by certain Acetobacter strains, resulting in higher yields.A study has demonstrated the remarkable efficiency of phosphofructokinase in Acetobacter, which catalyzes the conversion of fructose-1-phosphate to fructose-1,6-bisphosphate 63 .In another study, Gluconoacetobacter hansenii  was evaluated for cellulose production using different carbon sources, including glucose, fructose, inulin, and mannitol.The highest cellulose yield was obtained when fructose was used as the sole carbon source 64 .While it was found that media containing sucrose from subsidized coconut juice was the best media for cellulose production by A. xylinum 65 , it was found that higher cellulose production by A. xylinum ATCC 10245 bacteria was obtained when glycerol was used as the carbon source.The consumption rates of the carbon sources affected the amount of cellulose product, not only the type 66 .Using both carbon sources, mannitol, and arabitol, resulted in high amounts of cellulose by A. xylinum in static cultures 67 .

Determination of the optimal glucose concentration for BC production
The effects of different glucose concentrations on cellulose production by Rhizobium sp. are shown in Fig. 2B.The addition of glucose to the cellulose production media at a concentration of 1.5% resulted in the production of 2.05 g/L.Cellulose productivity decreased when the glucose concentration increased by 3% and reached 1.52 g/L, whereas a concentration of 4% reached 0.35 g/L.This was probably caused by oxidizing a large amount of glucose, causing it to accumulate in large quantities.The acidity of gluconic media increases due to inhibition of cellulose production.A decrease in the amount of cellulose produced by K. hansenii increases the glucose concentration in the production media by 4% 64,68,69 .

Determination of the optimal nitrogen source for BC production
The effects of different nitrogen sources on cellulose production by Rhizobium sp. are shown in Fig. 2C.Compared to other nitrogen sources, yeast extract showed the highest cellulose productivity.This can be explained by the fact that yeast extract contains significant concentrations of essential vitamins and specific growth hormones.The amount of cellulose produced was 2.2 g/L, followed by peptone at 0.8 g/L and tryptone at 0.56 g/L.Therefore, yeast extract was chosen as the nitrogen source for cellulose production in subsequent experiments because NH 4 Cl and (NH 4 ) 2 SO 4 did not yield sufficient results.

Determination of the optimal concentration of yeast extract for BC production
The effects of different yeast extract concentrations on cellulose production by Rhizobium sp. are shown in Fig. 2D.It was found that 2.17 g/L of cellulose was produced when yeast extract was added to the media at a concentration of 0.05%.An increase in cellulose productivity was observed when the concentration of yeast extract was increased by 0.1%, and reached 2.22 g/L when the concentration of 0.15% reached 2.27 g/L, and decreased when the concentration reached 0.2% reached 2.10 g/L.

Environmental conditions
pH value pH is an important factor in the control of the oxidative fermentation process for BC production.An acidic or near-neutral pH environment is considered to be optimal for the production of BC 70 .Figure 3 illustrates the impact of pH on cellulose production by Rhizobium sp., employing a carbon source (glucose) at a concentration of 1.5% and a nitrogen source (yeast extract) at 0.15%.The manipulation of pH from 5.5 to 6.5 positively influenced bacterial cellulose production, with the optimal outcome achieved at pH 6.5, yielding 2.5 g/L.

Temperature
Temperature stands out as a crucial factor capable of shaping an organism's adaptation strategies for survival by impacting its regular homeostatic functions 70 .The optimum temperature of 30 °C was used to obtain the maximum yield of cellulose produced by Rhizobium sp.The amounts of cellulose produced were 2.21 g/L at 30 °C and 1.65 g/L at 35 °C.Temperature is a crucial variable affecting the growth and production of cellulose.
Extensive research has shown that the ideal temperature range for cellulose production is 25-30 °C64 .Several studies have shown that the maximum cellulose yield ranges from 28 to 30 °C71 .

Aeration
The amount of cellulose produced in the flask covered with cotton was 2.5 g/L, whereas that produced in the uncovered flask was 2.03 g/L.The aerated cultures were examined to determine the effects of carbon dioxide and oxygen pressure.A previous study showed that the rate of cellulose production did not depend on the increase in the pressure of the oxygen.However, the production rate was dependent on the oxygen transfer rate, which decreased with an increase in the viscosity of the broth.This reduction in rate was attributed to the high carbon dioxide pressure.However, this decrease was reversed by a constant increase in the rate of airflow 72 .

Characterization of BC/K.h, BC/K.h-Nis, BC/Rhiz, and BC/Rhiz-Nis
The thickness of BC/K.h,BC/K.h-Nis,BC/Rhiz, and BC/Rhiz-Nis The thickness of the pure BC/K.h membrane measured 35 µm when wet and 10 µm when dry.In the wet state, the BC/K.h-Nismembrane exhibited a thickness of 42 µm, reducing to 13 µm when dry.The pure BC/Rhiz membrane's wet state thickness was 3 mm, aligning with the 10 µm thickness observed in dry conditions.The BC/Rhiz-Nis membrane displayed a wet state thickness of 34 µm, diminishing to 11 µm when dry.A visual representation of the results and sample details for the BC composite membranes can be found in Fig. 4 and Table 2, respectively.

FTIR analysis of BC/K.h, BC/K.h-Nis, BC/Rhiz, and BC/Rhiz-Nis membranes
In this study, FTIR analyzes BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis membranes were performed to verify the synthesis of BC/K.h,BC/K.h-Nis,BC/Rhiz, and BC/Rhiz-Nis composites.The FTIR spectra of the nanocomposites of BC, nisin, and BC/Nis are shown in Fig. 6.The -OH functional group showed characteristic peaks at 3372/cm in the FTIR spectra of pure BC.Similarly, peaks corresponding to C-H stretching vibrations were observed at 2900 and 1620/cm.Moreover, the characteristic peaks for the C=O group were observed at 1420 and 1100/cm.As previously reported 73,74 , significant absorption bands associated with hydroxyl and amino acid functional groups were also observed for pure nisin.
In the 3302/cm region, vibrations originated from the O-H bond of pure nisin.In the FTIR spectra, the band corresponding to the absorption of the carbonyl (C=O) stretching of the secondary amide (amide I band) was detected at 1600.5/cm.In addition, peaks for the bending vibrations of the (C=O) were obtained at 1500.3/cm.Characteristics of BC/K.h-Nis composite clearly shows that the absorption peak for the -OH bending vibration occurs at 1028/cm for cellulose due to the presence of water molecules.The absorption peaks of nisin (amide II and N-H bending vibrations) appeared at 1642 and 1588/cm 75 .Owing to the dehydration of BC, the peak disappeared at 3424/cm.These results indicate that nisin interacts well with BC.Similar spectra were obtained for the BC/Rhiz-Nis.

WHC and WRR of BC/K.h, BC/K.h-Nis, BC/Rhiz, and BC/Rhiz-Nis membranes
For biomedical applications of BC, WHC and WRR are essential properties.WHC and WRR are directly related to changes in the BC matrix's surface area and pore size.The porous and fibrous nature of BC is responsible for its high WHC.According to 76 , hydrogen bonds hold water in pores and cellulose fibrils.The pore sizes of the BC composites (BC/K.h-Nisand BC/Rhiz-Nis) were smaller than those of pure BC, as shown by the WHC and WRR results of this study.WHC of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis were 115, 120, 130, and 126 times their dry weights, respectively.
The difference in pore size contributed to the increased WHC rates of the two composites compared to pure BC.As shown in Fig. 7A and B, the WHC of the composites was higher than that of the pure BC.These composites have smaller pore sizes, which lead to enhanced binding of the penetrating water molecules between the microfibrils.This led to a longer residence time for the water molecules in the BC fibrils of the composites.In comparison, the WRR obtained using pure BC is higher.The more space in the BC matrix, the more water can penetrate the material; however, water evaporates faster.Therefore, a larger pore size leads to higher WRR in BC samples 77 .Another study showed that changes in the physical properties of BC, such as WHC and WRR, were associated with changes in various parameters, such as microfibril arrangement, pore size, pore volume, and surface area following structural modifications 78 .
In summary, pore size, fibril arrangement, and pore volume have an influence on the WHC and WRR.In addition, modifying pure BC with nisin resulted in the restructuring of BC fibrils, leading to an improved water absorption capacity.

The porosity analysis of BC/K.h, BC/K.h-Nis, BC/Rhiz, and BC/Rhiz-Nis membranes
The porosity of the membrane is quantified as the fraction of the void volume within the membrane, which is precisely calculated by dividing the volume occupied by the pores by the total volume enclosed by the membrane 79 .Porosity of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis were 60.5%, 54.4%, 57.8%, and 50.3%, respectively.The results are shown in Fig. 8A.Our experimental results are consistent with the findings of dos Santos et al. 80 ; when examining the X-ray microtomography parameters of BC and BC-Nis membranes, it was observed that BC membranes exhibited greater connectivity compared to the BC-Nis membranes.Furthermore, the inclusion of nisin resulted in a 2% reduction in membrane porosity, which aligns with findings from SEM images indicating interconnected pores distributed evenly throughout the sample 80 .
Filtration analyses of BC/K.h,BC/K.h-Nis,BC/Rhiz, and BC/Rhiz-Nis membranes A filtration study was performed to investigate the ability of the fluids to permeate the composites.Figure 8B shows the water permeation properties of the composite membranes.The results of filtration analyses for BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis revealed 24.18 mL/min, 18.4 mL/min, 22.33 mL/min, and 17.58 mL/min, respectively.Filtration capacity of BC/K.h-Nis,BC/Rhiz, and BC/Rhiz-Nis composite membranes were lower than BC/K.h.This can be attributed to the different physical properties of the composite membranes.The fibrous network of BC/K.h was spatially better arranged than those of the other composites (Fig. 5A).For example, the filtration capacity of BC/K.h-Nis is much lower than that of the other membranes.This is probably due to the tightly woven fiber network, which significantly reduces the filtration of the liquid yield compared to the other composites (Fig. 5B).However, similar structural properties are evident in the close numerical relationship between BC/K.h and BC/Rhiz compositions.Owing to their high hydrophilicity, BC/K.h and BC/Rhiz had higher filtration rates than BC/Rhiz-Nis and BC/K.h-Nis.Water molecules were selectively dissolved in the noncomposites (BC/K.hand BC/Rhiz) and diffused mainly through the BC layer, resulting in higher filtration rates.
Filtration capacities of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis were determined, and the results are shown below: • In the case of pure BC/K.h, the filtration time for 100 mL of distilled water was 4.01 min, resulting in a residual water volume of 97 mL.• The BC/K.h-Nis membrane required 5 min to filter 100 mL of distilled water, leaving a residual water volume of 92 mL.• For the BC/Rhiz membrane, the filtration time for 100 mL of distilled water was 4.3 min, with a residual water volume of 96 mL.Filtration is an essential and routinely used technique in practice.The objective or application typically determines the pore size of the filter.These include mycoplasma removal, laboratory sterilization, media filtration, biological fluids, gases, solutions, and solvents 81,82 .

Swelling analysis of BC/K.h, BC/K.h-Nis, BC/Rhiz, and BC/Rhiz-Nis membranes
The swelling ability of bacterial cellulose refers to the ability of the cellulose to absorb and hold onto water or other liquids.Bacterial cellulose typically has a high swelling ability due to its porous structure and hydrophilic nature 83 .Swelling abilities of BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/Rhiz-Nis were investigated to determine the ability of water to penetrate the structure (Fig. 8C).Swelling results for BC/K.h,BC/K.h-Nis,BC/Rhiz and BC/ Rhiz-Nis were 69%, 55.1%, 45.8%, and 35.6%, respectively.The results are presented in Table 2.According to 84 , swelling and crystalline linearity are directly proportional to the hydrophilicity/hydrophobicity of the material.
According to 84,85 , owing to the enormous hydrophilic properties of BC, water can easily penetrate cellulose and break the van der Waals force between the molecules, resulting in hydrogen bonds.The results showed that the swelling value of the K. hansenii cellulose product was higher than those of the other composites (BC/K.h-Nis,BC/Rhiz, and BC/Rhiz-Nis) due to its chemical and physical properties.Chemically, pure BC swells more than BC/Nis and BC/Rhiz because it is naturally hydrophilic and can absorb large amounts of water.Physically, BC has a highly porous fiber network with many interspersed and perforated voids.The BC composite (BC/K.h-Nis,BC/Rhiz, and BC/Rhiz-Nis) may have affected the physical properties of BC/K.h such that this fibrous network is impaired/reduced, and swelling values are ultimately lower than pure BC.
Swelling, which is influenced by several factors, is essential for understanding hydrogel structures.In the case of cellulose, swelling maintains the reticulated structure as part of particles, fibers, or as a film.However, the physical properties changed significantly, and the sample volume increased due to the swelling agent's absorption.However, the swelling of cellulose has a unique property: destruction of the supramolecular structure of cellulose.Thus, both processes were controlled using the same solvent and biopolymer.Therefore, depending on the properties of cellulose and operating conditions, there is no clear boundary between the swelling process and the same system 86 .

Conclusion
The remarkable versatility of BC as a biomaterial has led to its extensive use in developing high-quality paper, nanocomposites, wound dressings, and artificial vascular constructs.In this study, a novel BC producer, Rhizobium sp., was isolated from bean roots and evaluated for its ability to produce BC in simple, cost-effective media.In this study, the growth and BC production conditions were optimized for Rhizobium sp., and the BC produced by Rhizobium sp. was successfully modified with nisin, which exhibits broad-spectrum inhibitory activity against various microorganisms.The resulting BC was compared with the BC produced by K. hansenii.The results showed that BC produced by Rhizobium sp. had properties similar to those of BC produced by K. hansenii.
Moreover, BC-Nis composites showed remarkable inhibitory activity against E. coli and P. aeruginosa.These results suggest that BC production by Rhizobium sp. and its modification with nisin could be used in various industries.To improve BC production and shorten the production time, further molecular studies are required to isolate the genes responsible for BC production in Rhizobium sp. and improve their expression.In addition, the potential use of BC composites produced by Rhizobium sp. and other materials should be investigated for various applications in bioelectronics, medicine, agriculture, and the food industry.Overall, this study provides valuable insights into the production and modification of BC by Rhizobium sp. and its potential applications in various fields.

Figure 2 .
Figure 2. The effect of different concentrations of carbon sources (A), glucose (B), nitrogen sources (C), and yeast extract (D) on the production of cellulose in static culture (for nitrogen sources and yeast extract, glucose concentration was 1.5% in static culture).Letters indicate significant differences P < 0.05 when comparing different treatments.

Figure 3 .
Figure 3.Effect of pH on cellulose production with glucose concentration (1.5%) and yeast extract concentration (0.15%) in static culture.The letter indicates significant differences P < 0.05 when comparing different treatments.
, BC/Rhiz, and BC/Rhiz-Nis membranes FE-SEM was used to analyze the structure of lyophilized samples of BC/K.h,BC/K.h-Nis,BC/Rhiz, and BC/ Rhiz-Nis membranes.The surfaces of the lyophilized samples were examined for comparative analysis.The results are shown in Fig.5.The cellulose microfibrils in pure BC/K.h were randomly distributed and contained many voids, as shown in Fig.5A.

Table 1 .
Biochemical test results for Rhizobium sp.